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Who Discovered SPME? Solid Phase Microextraction was invented in 1990 by Dr. Janusz Pawliszyn and his colleagues from the University of Waterloo in Canada. He invented this technique to “address the need for a fast, solvent-free, and field compatible sample preparation method”, which faster and more efficient is the name of the game in industry.

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What is an SPME? It consists of coated fibers that are used to isolate and concentrate analytes into a range of coating materials. After extraction, the fibers are transferred to an analytical instrument for separation and quantification of the target analytes. This is accomplished with the help of a syringe-like handling device that protects your sample while transferring from your sample to the instrument. This syringe-like device also protects your fiber during storage. SPME, also known as “Spee Mee”, is a solvent-free adsorption/desorption technique.

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More on SPME SPME is also a microextraction technique that, when compared to the sample volume, contains a very small amount of extraction solvent. SPME allows for an equilibrium to be reached between the sample matrix and the extracting phase rather than an exhaustive removal of the analytes to the extracting phase occurring. –The extracting phase is permanently attached to a rod that is made out of different materials, which makes this approach practical. The amount of analyte adsorbed by the fiber depends on the thickness of the coating and on the distribution constant of the analyte. Extraction time depends on the length of time required to obtain precise extractions for the analytes with the highest distribution constants. Selectivity can be changed by altering the type of fiber used to match the characteristics of the analytes of interest. –Volatile compounds require a thick coating and semivolatile analytes a thin coating.

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How does SPME work? First, you draw the fiber into the needle. The needle is then passed through the septum that seals the vial. You then depress the plunger to expose the fiber to your sample or headspace above the sample. Organic analytes are then adsorbed to the coating on the fiber. After adsorption equilibrium is attained, which can be anywhere from 2 minutes to 1.5 hours, the fiber is drawn back into the needle and is withdrawn from the sample vial. Finally, the needle is introduced into the GC injector or SPME/HPLC interface, where adsorbed analytes are thermally desorbed and delivered to the instruments column.

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Reaching Equilibrium The extraction is considered to be complete when it reaches equilibrium and the conditions can be described by the following equation: This equation shows the relationship between the analyte concentration in the sample and the amount extracted by the coated fiber. If the amount of analyte extracted onto the fiber is an insignificant portion of that present in the sample, this equation simplifies to n=K fs V f C 0, where the amount of extracted analyte is independent of the volume of the sample. This means that: there is no need to collect a defined amount of sample prior to analysis the fiber can be exposed directly to whatever is being analyzed and the amount of extracted analyte will correspond directly to its concentration in the matrix This allows for the prevention of errors associated with the loss of analyte through decomposition or absorption onto sampling container walls.

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Other SPME holders available SPME Portable Field Sampler Contains an internal septum that stores your fiber after sampling by sealing it. Great for field work Comes with – a PDMS/Carbowax fiber for trace-level volatile analysis –Or a PDMS fiber for concentrating polar analytes This holder is used with an autosampler or an SPME/HPLC interface…requires an upgrade kit for autosampler use. Contains a needle that moves freely for control by an automated system, and for depth regulation in the interface desorption chamber.

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StableFlex Fibers These type of fibers are coated on a flexible fused silica core instead of the standard fused silica core used on the other fibers. This coating partially bonds to the flexible core which results in: – a more stable coating –a more durable and longer lasting fiber These special coated fibers are for GC use only. They also have the same temperature, conditioning, and cleaning requirements as the other fiber of its same coating and thickness. These are available in every coating EXCEPT for PDMS, Polyacrylate, and CW/TPR.

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Carbowax/Templated Resin (CW/TPR) Film ThicknessDescription Hub Description Recommened use 50μm* Partially crosslinked Purple/plain Surfactants on HPLC * This fiber is more durable due to it not containing any epoxy

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Maintenance on SPME Chlorinated solvents my dissolve the epoxy that holds the fiber so DO NOT USE CHLORINATED SOLVENTS EVER. Use caution when handling PDMS/DVB and CW/DVB fibers because the coating can be inadvertently stripped off. Cleaning your fiber depends on the fiber phase coating: –Bonded can be taken to maximum temperature and thermally cleaned for 1 hour to overnight, or can be rinsed in an organic solvent and then thermally cleaned. –Non-bonded can only be thermally cleaned and can be taken to the maximum temperature for 1 to 2 hours or baked overnight at degrees under the maximum temperature. If not clean after this treatment, thermally treat it for 30 minutes at 20 degrees above the maximum temperature. –Partially bonded fibers can be rinsed in water-miscible organic solvents.

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Sampling with SPME Consistent sampling time, temperature, and fiber immersion depth are crucial to this technique when it comes to high accuracy and precision. Equilibrium is attained more rapidly in headspace than in immersion because the analytes can diffuse more rapidly to the coating on the fiber. The thicker the fiber coating, the more analytes that are extracted, which is proven in the figure below.

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Injecting and Running a Sample on GC This is where you inject your SPME needle on the GC-MS

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Advantages of SPME During desorbtion of the analyte, the polymeric phase is cleaned and ready for reuse. Absence of solvent makes SPME –environmentally friendly –separation is faster –throughput increases and allows for use of simpler instruments Small in size –great for field work. –Amount of extracting phase is small and equilibrium of system is not disturbed –Very small objects can be studied High sensitivity and limit of determination All extracted analytes are transferred to the analytical instrument Can sample directly into a sample or the headspace above sample. Range of analytes that can be analyzed include volatile, semivolatile, nonvolatile, and inorganic species. coupled with other instruments besides GC like CE, LC, and MS. When compared to similar extraction methods, SPME has a better detection limit, precision, cost, time, solvent use, and simplicity, which is shown in the table below.

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Disadvantages of SPME Can get relatively expensive if one is not careful with fibers due to the cost being roughly $108 per fiber. Polymer coating is fragile, easily broken, and have limited lifetime. Also a monopoly with Supelco being the only suppliers of the fibers so cost continuously increases. Its main limitation is its reduced concentration capability due to the small volume of polymer coating on the fiber, which is being addressed and researched further by Dr. Pawliszyn.

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Why SPME? It can be used to analyze various types of analytes from gaseous, liquid, and solid samples instead of specializing in just one type like LLE or Headspace. Very cheap compared to other extraction methods. Reduces sample preparation times and disposal costs due to being solvent-free, also a bonus for the environment. Improves detection limits. A very simple methods that almost anyone could perform.

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Different fields using SPME Applications SPME is applied to include: –Food and drug –Environmental –Clinical/Forensics

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Choosing Best Sample Preparation Technique Sample preparation constitutes for over 80% of your total analysis time so an effective sample is desired, especially by the food and drug industry where time is money. The following is desired in sample preparation of pharmaceuticals: –Loss of very little sample –Good yield recovery of analyte of interest –Coexisting compounds removed efficiently –Procedure can be performed conveniently and quickly –Cost of analysis is kept to a minimum

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Comparing Extraction Methods for Pharmaceutical Analysis SPE and LLE in drug analysis: Both complicated and time-consuming, which limits the number of samples Prone to sample loss due to being multi-step Require large sample amount Require an organic solvent Difficult in automating these procedures Additional cost for waste treatment SPME, as we have heard in previous slides, prevents all of these common drawbacks listed for SPE and LLE.

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SBSE Stir bar sorptive extraction, or SBSE, is a very similar technique to SPME. It is a technique that is used for the analysis on both volatile and semivolatile organic compounds in aqueous environmental samples. When compared to SPME, SBSE has higher recoveries and higher sensitivity. The extraction is performed by placing the stir bar in the sample for minutes. –After extraction, stir bar is placed in a glass thermal desorption tube that is placed in a thermal or liquid desorption unit to be thermally desorbed and analyzed.

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In-Tube SPME These compounds are then desorbed by introducing a stream of mobile phase, or by a static desorption solvent when analytes are more strongly adsorbed to capillary coating. Desorbed compounds are then injected into the LC or HPLC column for analysis. Filtering sample solution before extraction should by performed to prevent plugging of capillary column and flow lines. Extraction yields are generally low, but compounds are reproducible when using an autosampler. This technique uses an open tubular capillary as an SPME device. Can be coupled on-line with HPLC or LC/MS which is represented in the provided diagram. In aqueous samples, a direct extraction from sample into coated stationary phase of capillary is performed.

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Solid-Phase Dynamic Extraction (SPDE) Trapped analytes are then recovered by heat desorption directly into a GC injector body, which was shown to you in a previous slide. A great advantage of this technique over SPME is the robustness of the capillary and the fact that it is nearly impossible to damage this mechanically. This has been used to analyze volatile compounds, pesticides, and some drugs successfully. The only drawback to this technique is that it tends to have carryover because the analytes tend to remain in the inside needle wall after heat desorption. This technique is for vapor and liquid samples. Dynamic sampling is performed by passing the headspace through the tube using a syringe. They analytes are then concentrated onto PDMS and activated carbon, which are coated onto the inside wall of the needle. This technique permits operation under dynamic conditions while keeping the headspace volume constant.

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More Results from Pharmaceutical Studies with SPME-Urine treated with drugs

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Clinical/Forensic Application This figure was an on-fiber derivitization for determination of fluoroacetic acid from blood. Pyrenyldiazomethane (PDAM) was loaded onto the fiber from n-hexane solution in the washing station of the sample. During headspace extraction, acid was on- fiber-transformed into pyrenylmethyl fluoroacetate, which was then measured by GC-MS with high sensitivity. Used for the detection and quantitative determination of illicit and therapeutic drugs, pesticides, solvents, and other poisons from blood, urine, hair, and human tissue. Samples were brought into a homogeneous aqueous solution by pretreatment of homogenization, protein precipitation, or centrifugation. Hair is first digested by NaOH or extracted with a suitable solvent. SPME conditions were determined by structure and properties of the analyte.

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List of Forensic Toxicology Applications

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List of Forensic Toxicology Applications cont’d

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Gadgets used in Forensics that are associated with SPME TuffSyringe TS100 This device preserves sample and prevents contamination of SPME fiber as well as inadvertent operation. Cost of this device is $245. SafePorter SP200/SP201 This transports/stores SPME holders and is constructed of machined aluminum that allows for the sample/holder to remain safe even if run over by a car. It also contains a dual o-ring that creats a hermetic seal to preserve and protect SPME holder/sample. Cost of the SP200 (comes with a septum) is $145 and the SP201 (without septum) is $135. Conditioner 1X This precisely measure and controls temperature from 0° to 350 ° and can clean other needles/syringes in addition to SPME fibers. Cost of this device is $1875.

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Environmental Application Air sample –Analytes are extracted by the fiber wither by direct exposure or by use of the headspace method. –Most applications involve the use of a commercial SPME fiber, but a dialuminum trioxide-coated fiber has been used for VOC sampling. –On-site air sampling can be performed by the equilibrium methods or by the non-equalibrium method, with quantification by use of calibration plots from a standard gas generating system of standard gas mixture as opposed to using equations. –rapid air sampling can be performed with controlled air-flow rate and quantified by use of diffusion- based calibration methods by use of wither the interface or cross-flow model. Water samples –Can be performed by direct immerion (DI), headspace (HS), or in-tube method. –The air inside needle must be completely replaced by water and effects of extracted analytes on the external wall of the needle should be avoided. –The in-tube SPME has been used for analysis of BTEX, PAH, pesticides, and herbicides in aqueous samples. –The fibers have also been used to analyze environmental pollutants in aqueous samples and have been accompanied by ultrasounds or microwaves. –Traditional calibration methods have been used for most applications, but diffusion-based calibration methods have been used. Soil and sediment samples –Performed by HS or DI methods and applications have been assisted by sonication, microwaves or by heater or cooling fiber. –Traditional calibrations but some exhaustive calibration methods have been used in quantification of BTEX in soil samples. –A hollow-fiber membrane-protected SPME has also been used for determination of herbicides in sewage-sludge samples.

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List of Environmental Applications -gas

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List of Environmental Applications-aqueous

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List of Environmental Applications-soil/sediment

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Some of My Results Results from black fiber Results from red fiber

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Conclusion SPME is a solvent-free microextraction technique that is: –Cost efficient –Simple to understand and use –High sensitivity –Low detection limits –Can be used to sample analytes of many types –Used in many areas of industry